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首页> 外文期刊>Indian Journal of Biotechnology >Regeneration of Biophytum sensitivum (Linn.) DC. through organogenesis and somatic embryogenesis
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Regeneration of Biophytum sensitivum (Linn.) DC. through organogenesis and somatic embryogenesis

机译:敏感生物phyphyum(Linn。)DC的再生。通过器官发生和体细胞胚发生

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A protocol was established to regenerate Biophytum sensitivum (L.) DC. through indirect and direct organogenesis and somatic embryogenesis. In the present study, MS medium supplemented with 2,4-D or NAA in combination with BAP induced callusing in stem, inflorescence tip and flower bud explants. MS amended with BAP caused callusing in stem and flower bud explants but failed to cause callusing in inflorescence tip explants. Calli obtained on 2, 4-D or BAP amended media produced multiple shoots upon subculturing on BAP (1.0 mg L super(-1)). When a combination of NAA (0.5 mg L super(-1)) + BAP (2.0 mg L super(-1)) was used calli obtained from stem, inflorescence tip and flower bud explants produced multiple shoots. In case of direct organogenesis, only inflorescence tip explants produced multiple shoots on MS medium supplemented with BAP. BAP at 3.0 mg L super(-1) induced maximum (50%) response. Regenerated shoots rooted on half strength MS medium supplemented with NAA 0.5 mg I super(-1). MS medium supplemented with 2, 4-D (2.5 mg I super(-1)) induced embryogenic response in calli from inflorescence explants. Embryogenic calli produced embryoids upon transfer to MS medium supplemented with NAA (1.0 mg L super(-1)) + BAP (3.0 mg L super(-1)). Embryoids were germinated on half strength MS medium. Eighty per cent of the rooted plantlets and 90% of somatic embryo derived plantlets survived on soil medium.
机译:建立了一个协议,以再生Biophytum敏感iv(L.)DC。通过间接和直接的器官发生和体细胞胚发生。在本研究中,添加2,4-D或NAA的MS培养基与BAP组合可诱导茎,花序尖端和花芽外植体中的愈伤组织。 MS用BAP改良后,在茎和花芽外植体中引起愈伤组织,但在花序尖端外植体中未引起愈伤组织。在2、4-D或BAP改良培养基上获得的愈伤组织在BAP(1.0 mg L super(-1))上继代培养后产生了多个芽。当使用NAA(0.5 mg L super(-1))+ BAP(2.0 mg L super(-1))的组合时,从茎中获得的愈伤组织,花序尖端和花芽外植体产生了多个芽。在直接器官发生的情况下,只有花序尖端外植体在补充有BAP的MS培养基上产生多个芽。 BAP在3.0 mg L super(-1)时诱导最大(50%)反应。再生芽生于半强度MS培养基中,该培养基中添加了NAA 0.5 mg I super(-1)。 MS培养基中添加了2,4-D(2.5 mg I super(-1)),诱导了来自花序外植体的愈伤组织的胚发生反应。胚胎发生性愈伤组织在转移至补充有NAA(1.0 mg L super(-1))+ BAP(3.0 mg L super(-1))的MS培养基后产生胚状体。胚状体在半强度MS培养基上萌发。 80%的生根小植株和90%的体细胞胚衍生小植株在土壤培养基上存活。

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